Title: Preparation of Large Epoxy Sections for Light Microscopy as an Adjunct to Fine-Structure Studies
Abstract: Tissue blocks 2 × 2 × 0.4 cm were fixed 6-24 hr in phosphate-buffered 5% glutaraldehyde then sliced to 2 × 2 × 0.1 cm and soaked in 0.1 phosphate-buffer (pH 7.3) for at least 12 hr. Fixation was continued for 2 hr in phosphate-buffered 1-2% OsO4. The slices were dehydrated, infiltrated with Araldite, and embedded in flat-bottomed plastic molds. Sectioning at 1-8 μ with a sliding microtome was facilitated by addition of 10% dibutylphthalate to the standard epoxy mixture. The sections were spread on warm 1% gelatin and attached to glass slides by drying, baking at 60 C, fixing in 10% formalin or 5% glutaraldehyde and baking again. Sections were mordanted in 5% KMnO4 (5 min), bleached with 5% oxalic acid (5 min) and neutralized in 1% Li2CO3 (1 min). Several stains could then be applied: azure B, toluidine blue, azure B-malachite green, Stirling's gentian violet, MacCallum's stain (modified), tribasic stain (modified) and phosphotungstic acid-hematoxylin. Nuclei, mitochondria, specific granules, elastic tissue or collagen were selectively emphasized by appropriate choice of staining procedures, and cytologic detail in 1-3 μ sections was superior to that shown by conventional methods. Selected areas from adjacent 4-8 μ sections could be re-embedded for ultramicrotomy and electron microscopy.
Publication Year: 1965
Publication Date: 1965-01-01
Language: en
Type: article
Indexed In: ['crossref', 'pubmed']
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Cited By Count: 67
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